A phytin-containing solution such as corn steep liquor, acid extract of rice bran is treated with an anion exchange resin with phytin adsorption. The phytin is then separated from the resin by alkali-elution, then the phytin thus recovered is further subjected to the treatment of hydrolysis under pressure, phosphate removement, purifying, etc. to prepare inositol. Alternatively, the recovered phytin is further subjected to the treatment of desalting, purfiying, etc. to prepare phytic acid.
|
1. A process for obtaining phytin or a product related to phytin, said process comprising:
(i) contacting a phytin-containing solution with an anion-exchange resin at a ph of 1-5 for a period of time sufficient for adsorption of at least part of the said phytin onto the said anion-exchange resin; and (ii) eluting phytin from the said anion-exchange resin.
2. The process of
(iii) recovering the said phytin from the eluate.
3. The process of
(iv) desalting and purifying the recovered phytin to obtain phytic acid.
6. The process of
7. The process of
9. The process of
|
1. Field of the Invention
This invention relates to a method for preparing phytin and related products including inositol and phytic acid.
2. Discussion of the Background
Phytin is a calcium magnesium salt of phytic acid. It is distributed in almost all parts of plant tissue, especially in seeds. It is an important source for producing inositol or phytic acid, both of which are used in the food industry. Phytic acid is a hexaphosphoric acid ester of inositol. It has a chelating action by which trace metals in foodstuffs are inactivated, preventing the discoloration and deterioration of foodstuffs.
Inositol is also called mesoinositol or myoinositol. It is contained in plants as a component of phytin, and is found in the free state in animal tissues such as muscle, heart, liver, etc. Inositol is also a component of phosphatides which is widely distributed in natural organisms, especially in mammalian liver and brain, egg yoke, soybean and wheat germ. It is important as a vitamin in the higher animals and performs an important role in the metabolism of fats and cholesterol. A number of studies have shown its lipotropic function, and its effect on cirrhotic livers and hyper-cholesteremia. Inositol has therefore recently become an important substance in the field of health foods in the United States and the other countries.
Inositol is usually produced from raw materials such as rice bran or corn steep liquor. For example, rice bran may be treated with an organic or inorganic acid to extract phytin. Phytin is then precipitated and separated from the extract, usually by filtration, to remove unwanted proteins and carbohydrates. The separated phytin is then hydrolyzed under pressure to recover inositol, which is further purified, concentrated, and crystallized. In this method, organic solvents, water-soluble metallic salts such as iron chloride, manganese sulfate, and water-soluble alkaline substances such as sodium hydroxide, aqueous ammonia, may be employed as precipitants for phytin. However, phytin usually precipitates as a colloidal, pasty substance when these precipitants are used, rendering satisfactory elimination of impurities extremely difficult.
Phytin may also be precipitated with calcium compounds such as calcium phytate. However in this case a large amount of proteinous, difficult to remove, impurities co-precipitate. Calcium phytate itself precipitates as a pasty crystallized mass. This often causes process problems, such as blocking of the nozzles of centrifugal separator during the operation. And a large amount of fine crystallized calcium phosphate forms as a by-product after the phytin hydrolysis step. A considerable amount of inositol is thus lost in this crystalline material in the successive inositol-calcium phosphate separating step, resulting in an unavoidable economic disadvantage due to a decrease in inositol recovery. The separated calcium phosphate is also unsatisfactory from an economical viewpoint due to its low purity.
There is thus a strongly felt need for a facile process for the production of phytin and related products in high yields and in high degrees of purity.
Accordingly, it is an object of this invention to provide a process for producing phytin and related products, e.g. inositol, phytic acid in high yields.
It is another ojbect of this invention to provide a process for producing phytin and related products, having a high degree of purity.
It is another object of this invention to provide a process for the facile production of phytin and related products.
It is another object of this invention to provide an economically advantageous process for the production of phytin and related products, e.g. inositol and phytic acid.
It is another object of this invention to provide a process for the production of pure phytic acid or inositol by further treatment of the phytin obtained.
The present inventors have now surprisingly discovered a novel process which satisfies all of the above objects of this invention, and other objects which will become apparent from the description of the present invention given herein below. In accordance with the invention, phytin is first adsorbed onto an anion exchange resin. It is then separated from the anion exchange resin by alkali elution. This method excludes the phytin precipitation step. The level of impurities contaminating the product is decreased, and the whole process is simplified. High purity phytic acid can be readily obtained from the phytin, using any known treatment method, such as desalting. The phytic acid can be further treated to prepare high purity inositol using any known treatment such as hydrolysis under pressure, separation of phosphates, and purification.
This invention provides a method for preparing high purity phytin in a simplified and an economical process. This invention also provides a method for preparing pure phytic acid and/or inositol by further treatment of the phytin obtained.
Phytin is extracted with organic or inorganic acid in a known manner and under known conditions from a phytin-containing raw material such as rice bran, wheat bran, or corn. Defatted rice bran is a good source for inositol preparation, from which phytin is extracted by 1% aqueous sulfuric acid solution. Corn steep liquor which is a steep water of corn grain in a dilute aqueous sulfur dioxide solution obtained by a corn wet-milling process, is also an acid extraction of phytin. It is a practical source for inositol preparation. It contains phytic acid or its salts in an amount corresponding to 2% (on a dry basis) of inositol.
The phytin-containing solution thus obtained is first contacted with a bed of anion exchange resin which adsorbs the phytin. Anion exchange resins useful for this purpose may be CO3, CH3 COO, Cl, SO3, OH, etc. type resins. Although any resin may be used, some resins vary from each other on the basis of their phytin-adsorbability, selectivity, effect on removing impurities, and the other characteristics. There are some differences between the types of the resin on the yield of phytin and the other effects. Practically speaking, Cl and SO3 type resins are preferable for this purpose. OH type resins are also suitable. Useful commercially available resins are, for example, Amberlite IR-45, IRA-68, IRA-93, IRA-410, and IRA-411, which are produced by ORUGANO Co., Ltd., Daiya-ion; and SA20A, SA21A, WA30, WA40, and WA11, which are produced by NIHON RENSUI Co., Ltd.; and Dowex MSA-1 and MSA-266, which are the produced by DOWEX Co., Ltd.
The conditions for the ion exchange resin treatment are usually selected within the following ranges: temperature =5 to 20°C, pH =1 to 5, concentration of phytin-containing solution =1 to 40% (w/v), flow rate, or space velocity (SV), for ion exchange resin (the amount of liquid fed to the resin per hour/volume of the resin) =0.5 to 20.
Phytin is adsorbed on the ion exchange resin by the above treatment. The resultant resin is then preferably washed preliminarily with hot water (t=30-85°C). The adsorbed phytin is then separated from the resin by alkaline elution. The alkaline substances which may be used for this purpose can be sodim hydroxide, potassium hydroxide, ammonium hydroxide and mixtures thereof. However the alkaline subtances which can be used are not limited to these particular examples. The elution conditions may vary according to the kind of alkali substance used, the concentration of their aqueous solution, the kind of ion exchange resin used, the properties of the phytin-containing solution, etc. In the case of sodium hydroxide, however, the following conditions are preferable: temperature =room temperature to 70°C; SV =0.5 to 10; and the pH of the eluted solution maintained between 9 and 12.
The eluted solution thus obtained contains mainly the sodium salt of phytic acid. The impurities in the solution, such as proteins, carbohydrates are present only in very low concentrations. Procedural difficulties in successive steps caused by these impurities are therefore considerably eliminated.
The eluted phytin solution is further subjected to the steps of hydrolysis under pressure, removal of the phosphates, purification concentration, and crystallyzation. Thus, an inositol product of high purity can be obtained with phosphates as a by-product. Sodium secondary phosphate will be obtained as a by-product when sodium hydroxide is used for elution. Alternatively, the eluted phytin solution is desalted by ion exchange resin to produce phytic acid.
By the process described above phytin is separated directly from a phytin-containing solution by a simple adsorption procedure. The troublesome treatment of a colloidal, pasty phytin precipitates found in conventional methods is completely excluded. Nearly all of the impurities remain in the original solution and do not contaminate the separated phytin. Thus, a highly purified inositol product and/or phytic acid product is produced very easily and economically.
Other features of this invention will become apparent from the following description of exemplary embodiments which are given for purposes of illustration, and are not intended to be limiting of the invention. EXAMPLE 1
Comparison of the method of this invention with a conventional inositol preparing process.
Phytin was separated by the methods given below using in each method 20 liters of corn steep liquor, and the inositol recovery and the protein content of the inositol were determined. The corn steep liquor used had pH of 4.1 and a concentration of 7.7%. It contained about 2% inositol.
Inositol recovery was calculated as follows: first an organic phosphor content observed in recovered phytin is calculated into phytic acid (C6 H18 O24 P6, molecular weight 660) equivalents, and then the phytic acid content thus obtained is calculated into inositol (C6 H12 O6, molecular weight 180) equivalents.
(1) Convention method
An aqueous 15% solution of calcium hydroxide was added to the corn steep liquor, adjusting the pH at 6.0 and precipitating phytic acid as its calcium salt. The precipitate was separated by filtration and washed with 1.5 liters of warm water (temperature ca. 50°C). 249 grams of phytin (as calcium salt), which is equivalent to 34.1 grams of inositol, were obtained.
(2) Method according to the present invention (1)
The corn steep liquor was passed through a bed of anion exchange resin at SV=4 with phytin adsorption. The resin used was 1 liter of OH type IRA-411 (produced by ORUGANO Co., Ltd.) which was regenerated to CO3 type before use.
The phytin-adsorbed bed of resin was washed by 1.5 liters of warm water (temperature ca. 50°C). Phytin was then eluted from the resin by passing a 7% aqueous sodium hydroxide solution through the bed of resin at SV=1. 115 grams of phytin was recovered as its sodium salt, which is equivalent to 115 grams of inositol (18.8 grams per a liter of resin).
(3) Method according to the present invention (2)
An anion exchange resin identical to that used in the preceding example (2) was regenerated to the CH3 COO type and treated with the corn steep liquor under the conditions used in example (1). 92 grams of phytin was recovered, which is equivalent to 16.5 grams of inositol per a liter of resin.
(4) Method according to the present invention (3)
An anion exchange resin IRA-68 of the OH type (produced by ORUGANO Co., Ltd.) was regenerated to the Cl type and treated with the corn steep liquor under the same conditions used in example (2). 212 grams of phytin was recovered, which is equivalent to 34.8 grams of inositol per a liter of resin.
(6) Method according to the present invention (5)
An anion exchange resin IRA-411 of the OH type was used for phytin recovery under the conditions used in example (2). 106 grams of phytin, which is equivalent to 17.3 grams of inositol per a liter of resin, was obtained.
The results obtained are tabulated below.
TABLE 1 |
______________________________________ |
Yield of crude |
Protein |
Method inositol (%) |
content (%) |
______________________________________ |
Conventional method |
94.2 73.5 |
Method of this 51.9 1.7 |
invention (1) |
Method of this 45.6 1.4 |
invention (2) |
Method of this 96.1 0.8 |
invention (3) |
Method of this 99.2 1.2 |
invention (4) |
Method of this 47.8 2.1 |
invention (5) |
______________________________________ |
NB (1) Yield of crude inositol: |
##STR1## |
(2) Protein content: |
##STR2## |
- As shown in Table 1, the protein content which represents impurities in |
phytin product is considerably lower in the products obtained by the |
method of this invention than in the product obtained by the conventional |
method. An anion exchange resin regenerated to the Cl or SO3 type |
apparently exhibits especially high yields of phytin recovery, which is |
shown as the yield of crude inositol in Table 1. |
150 liters of corn steep liquor (3.5 Baume and pH 4.1) containing 2.0 kg/m3 of inositol, calculated from phytin content, was passed through a bed consisting of 7.5 liters of anion exchange resin at SV=4 with phytin adsorption. The resin used was IRA-68 (produced by ORUGANO Co., Ltd.) which was regenerated to the Cl type with hydrochloric acid before use. The phytin-adsorbed resin was washed with a counterflow of warm water, then a 15% aqueous sodium hydroxide solution was passed through the resin at SV=1. About 12 liters of phytin-eluted solution was obtained.
The eluted solution was then concentrated to about 43 to 48% of sodium phytate content which is equivalent to 8.5 to 9.5% of inositol, and the concentrated solution was subjected to hydrolysis under pressure at 180°C for 3 hours. The resultant hydrolyzate was filtered to remove water-insoluble salts such as calcium phosphates, magnesium phosphates, etc., and the filtrate was subjected to a crystallizing procedure to separate the sodium secondary phosphate contained therein. The resultant inositol-containing solution thus obtained was decolorized and desalted by ion exchange resin and concentrated to around 25% inositol content. Inositol was crystallized out as its salt from the solution active carbon treatment, and some 250 grams of anhydrous inositol (moisture below 0.5%) was obtained by vacuum drying.
The amount of impurities contained in the product was very little.
About 5.6 kg of crystallized sodium secondary phosphate was obtained about 5.6 kg as a by-product in this process.
10 kg of defatted rice bran was extracted twice with an aqueous solution of sulfuric acid, first with a 1% solution and secondly with a 0.3% solution. The whole extracted solution volume of about 100 liters was treated by the same anion exchange resin used in Example 2 at SV=2.
The phytin adsorbed resin was washed with warm water and eluted with a 10% aqueous solution of sodium hydroxide at SV=1. The recovered sodium phytate solution was about 15 liters, and about 206 grams of refined anhydrous inositol was obtained using the treatment of Example 2.
A liquid containing 100 ml of 35% hydrochloric acid in 13 liters of corn steep liquor was subjected to treatment with 1 liter of anion exchange resin of the OH type (Amberlite IRA-93) at SV=2.
About 22 grams of refined inositol was obtained by a treatment identical to that of Example 2.
Eluted solutions of sodium phytate obtained in the same manner as described in Examples 2 and 3 were treated for desalting 4 liters of OH-type cation exchanger (Amberlite IR-120B; DAIYA-ION SKlB and Dowex 88 are also available) at SV=2. The solution was concentrated to about 55% and decolored by active carbon.
1,340 grams of high quality, 50% phytic acid was recovered.
Obviously, numerous modifications and variations of the present invention are possible in light of the above teachings. It is therefore to be understood that within the scope of the appended claims, the invention may be practiced otherwise than as specifically described herein.
Patent | Priority | Assignee | Title |
10160776, | Apr 08 2014 | GEA Mechanical Equipment GmbH | Method for acquiring one or a plurality of recyclable materials from seeds |
11484051, | Nov 01 2018 | Florida Food Products, LLC | Rice bran extract compositions |
11785970, | Nov 01 2018 | Florida Food Products, LLC | Method for treating meat and seafood products with rice bran extract |
5292537, | Nov 12 1992 | Bran Tec, Inc. | Method for stabilizing rice bran and rice bran products |
5574180, | Mar 14 1991 | Reilly Industries, Inc. | Process for recovering phytic acid, lactic acid or inositol |
5593855, | Dec 08 1992 | DOOSAN CORPORATION | Method of using yeast to recover phytin by precipitation from cornsteep liquor or light steep water |
7326549, | Mar 19 2001 | Cargill, Incorporated | Myo-inositol oxygenases |
Patent | Priority | Assignee | Title |
2112553, | |||
3410929, |
Executed on | Assignor | Assignee | Conveyance | Frame | Reel | Doc |
Feb 20 1986 | OGAWA, HIROSHI | SHOWA SANGYO CO , LTD | ASSIGNMENT OF ASSIGNORS INTEREST | 004690 | /0195 | |
Feb 20 1986 | KANNO, TOMOEI | SHOWA SANGYO CO , LTD | ASSIGNMENT OF ASSIGNORS INTEREST | 004690 | /0195 | |
Feb 20 1986 | OGAWA, HIROSHI | SHIKISHIMA STARCH MANUFACTURING CO , LTD | ASSIGNMENT OF ASSIGNORS INTEREST | 004690 | /0195 | |
Feb 20 1986 | KANNO, TOMOEI | SHIKISHIMA STARCH MANUFACTURING CO , LTD | ASSIGNMENT OF ASSIGNORS INTEREST | 004690 | /0195 | |
Feb 24 1986 | Showa Sangyo Co., Ltd. | (assignment on the face of the patent) | / | |||
Feb 24 1986 | Shikishima Starch Manufacturing Co., Ltd. | (assignment on the face of the patent) | / |
Date | Maintenance Fee Events |
Sep 07 1990 | M173: Payment of Maintenance Fee, 4th Year, PL 97-247. |
Sep 20 1990 | ASPN: Payor Number Assigned. |
Oct 21 1994 | M184: Payment of Maintenance Fee, 8th Year, Large Entity. |
Oct 07 1998 | M185: Payment of Maintenance Fee, 12th Year, Large Entity. |
Date | Maintenance Schedule |
May 26 1990 | 4 years fee payment window open |
Nov 26 1990 | 6 months grace period start (w surcharge) |
May 26 1991 | patent expiry (for year 4) |
May 26 1993 | 2 years to revive unintentionally abandoned end. (for year 4) |
May 26 1994 | 8 years fee payment window open |
Nov 26 1994 | 6 months grace period start (w surcharge) |
May 26 1995 | patent expiry (for year 8) |
May 26 1997 | 2 years to revive unintentionally abandoned end. (for year 8) |
May 26 1998 | 12 years fee payment window open |
Nov 26 1998 | 6 months grace period start (w surcharge) |
May 26 1999 | patent expiry (for year 12) |
May 26 2001 | 2 years to revive unintentionally abandoned end. (for year 12) |